Influence of Aqueous Phase Composition on Double Emulsion Stability and Colour Retention of Encapsulated Anthocyanins

Water-in-oil-in-water (W1/O/W2) emulsions (double emulsions) have often been used for the encapsulation of bioactive compounds such as anthocyanins. Instability of both anthocyanins and double emulsions creates a need for a tailored composition of the aqueous phase. In this work, double emulsions with a gelled internal water phase were produced and monitored over a 20-day storage period. The effect of the electrolyte phase composition (varying electrolyte components, including adipic acid, citric acid, and varying concentration of potassium chloride (KCl)) on anthocyanin and double emulsion stability was analysed using colour analysis, droplet sizing, and emulsion rheology. The effect of electrolytes on colour retention was shown to differ between the primary W1/O emulsion and the secondary W1/O/W2 emulsion. Furthermore, droplet size analysis and emulsion rheology highlighted significant differences in the stability and structural behaviour of the emulsions as a function of electrolyte composition. In terms of colour retention and emulsion stability, a citrate-buffered system performed best. The results of this study highlight the importance of strict control of aqueous phase constituents to prevent anthocyanin degradation and maximise double emulsion stability. Additional experiments analysed the effect of pectin chemistry on the anthocyanin colour retention and leakage, finding no conclusive difference between the unmodified and amidated pectin.


Introduction
Anthocyanins are a class of naturally occurring polyphenolic compounds responsible for the vibrant blue, red, and purple colours of many fruits and vegetables, which have also been used as a natural colourant in the food industry (where it is given the food colourant code E163 [1], and is authorised for use in the European Union, Australia, and New Zealand, and can be found in common supermarket products such as baked goods, chocolates, and energy drinks). Anthocyanins are also reported to have a number of health benefits including anti-cancer, anti-inflammatory, and anti-oxidant properties [2][3][4]. However, the colour and bioactivity of anthocyanins when deployed as food colourants are often diminished due to degradation and/or oxidation resulting from chemical and physical factors such as temperature, pH, and exposure to UV light, metal ions, and ascorbic acid [5][6][7][8]. As such, encapsulation methods are routinely employed to protect anthocyanins against degradation when prepared with different electrolyte compositions was investigated through colour analysis, particle size measurements, encapsulation efficiency, and rheological studies over 20 days. To the best of our knowledge, this is the first study to investigate the effect of electrolyte composition and pectin chemistry on both the physical stability of a double emulsion and the colour stability of the encapsulated anthocyanins.

Preparation of Water-in-Oil-in-Water (W 1 /O/W 2 ) Emulsions
Anthocyanin-loaded W 1 /O/W 2 emulsions were prepared using a two-stage emulsification process [15,22]. An initial anthocyanin-loaded water-in-oil (W 1 /O) emulsion was prepared, followed by the addition of a second water phase (W 2 ) and subsequent emulsification to produce the W 1 /O/W 2 emulsion. Four different background electrolyte solutions were used in this work: 0.1 M citrate buffer, 0.1167 M adipic acid, 0.35 M KCl, and 0.0075 M KCl (note: adipic acid was solubilised using a solution at slightly elevated pH, using the addition of potassium hydroxide, and then the pH was reduced to the value used in emulsion preparation). All electrolyte solutions were adjusted to pH 3.5 and contained 0.2 wt% potassium sorbate as an antimicrobial agent (even though the pH of all electrolytes was initially adjusted to 3.5, for KCl solutions the final pH values were higher once the final W 2 solutions were prepared (see Table S1)). The nature of the weak electrolytes means that the solution conductivity was used for comparison instead of ionic strength. The oil phase was prepared by adding 2.5 wt% PGPR to olive oil followed by stirring (using a stirring hotplate and magnetic stirrer bar) at 60 • C for at least 30 min to ensure complete dissolution. The W 1 phases were prepared by combining two separate solutions: a pectin solution and an anthocyanin solution. The 3.0 wt% pectin solutions were prepared by dissolving either amidated or unmodified pectin in the background electrolyte via stirring at 95 • C. Solutions of anthocyanin (40 mg/mL) were prepared by dissolving the extract in background electrolyte containing Ca 2+ ions at a concentration equal to 0.25 wt% (for amidated pectin) or 0.50 wt% (for unmodified pectin) of the total pectin mass (once the pectin and anthocyanin solutions were combined). These Ca 2+ concentrations yield a solution that flows at room temperature and gels upon cooling. Once pectin hydration/dissolution was complete, the solutions were cooled for 2 min before addition to the anthocyanin solution at a 1:1 weight ratio. W 2 phases were prepared by adding 1.5 wt% CMCNa and 1.5 wt% soy lecithin in background electrolyte and stirring at 60 • C until completely hydrated/dissolved. Primary W 1 /O (water fraction, ϕ W1 , of 30%) emulsions were prepared by adding 9 g of the combined W 1 phase to 21 g oil phase prior to emulsification at 20,000 rpm for 3 min using a Unidrive X 100 D rotor stator homogeniser (Ingenieurbüro CAT, Ballrechten-Dottingen, Germany). Emulsions were stirred briefly with a clean glass pipette before being homogenised for a further 1 min at 20,000 rpm. The prepared W 1 /O emulsions were placed in a fridge (T = 4 • C) for 1.5 h to ensure pectin gelation.
Secondary W 1 /O/W 2 emulsions (primary emulsion fraction, ϕ W1/O , of 30%) were prepared by adding 18 g of the W 1 /O emulsion (with a gelled internal W 1 phase) to 42 g of the W 2 phase. The two phases were then homogenised at 16,000 rpm for 3 min. Emulsions were placed into clean, amber glass vials, sealed with screw-top caps, and stored in the dark at 25.0 ± 0.1 • C in an incubator (Memmert GmbH + Co. KG, Büchenbach, Germany).
Each emulsion system was prepared in triplicate as independent repeats. The three independent emulsions were used in all subsequent experiments.

Emulsion Microstructure
Confocal laser scanning micrographs of a W 1 /O/W 2 emulsion (amidated pectin, 0.1 M citrate buffer system) diluted (1:1 w/w) in 0.1 M citrate buffer and stained with a lipid soluble fluorescent dye, Nile red (Sigma Aldrich, Castle Hill, Australia), were taken on days 1, 2, and 5. Ten µL of 1 mg/mL Nile red in ethanol solution was added to 300 µL of diluted emulsion and vortexed briefly (≈10 s). Approximately 2 µL of the diluted, stained emulsion was sandwiched between two clean, microscope cover slips (Gerhard Menzel GmbH, Brunswick, Germany). Images were taken using a Zeiss LSM 710 Elyra PS.1 microscope fitted with a water immersion objective, C-Apochromat 63×/1.2 W Korr M27 (ZEISS Group, Oberkochen, Germany). The excitation wavelength was 514 nm and the detection wavelength ranged from 539 to 753 nm.

Droplet Size Analysis
Emulsion droplet size distributions were determined using a Malvern Mastersizer 3000 equipped with a Hydro-LV sampling attachment (Malvern Panalytical, Malvern, UK). The Hydro-LV attachment was rinsed five times with Milli-Q water prior to and between samples, before being emptied and filled with the background electrolyte relevant to the emulsions being studied. The stirrer speed was kept constant at 1000 rpm and no sonication was used. The refractive indices of the oil and aqueous phases were set to 1.45 and 1.33, respectively, while the absorbance value was held at 0.01.

Colour Stability Measurements
Evaluation of the colour parameters over time was undertaken following the CIE L*a*b* parameters ( Figure S2, Supplementary Material) using a HunterLab UltraScan VIS spectrophotometer (Hunter Associates Laboratory Inc., Reston, VA, USA). The samples were placed in 10 mm quartz cuvettes (Starna Scientific, Baulkham Hills, Australia), placed in the instrument for light exposure, and reflected light was collected (at 8 • to the incident light angle). The a* (red-greenness), and b* (blue-yellowness) parameters were used to calculate chroma (c*) and hue angle (h • ) via Equations (1) and (2), respectively:

Emulsion Rheology
The rheological behaviour of the emulsions as a function of time and electrolyte composition was monitored using a Kinexus pro+ rotational rheometer (Malvern Panalytical, Malvern, UK). A cone and plate geometry (cone diameter of 40 mm, angle of 4 • , and a gap of 0.1584 mm) was used and all measurements were conducted at 25.0 • C. Strain sweeps were conducted in the range 0.1-100% with the frequency held constant at 1 Hz. Shear rate ramps were conducted from 1-100 s −1 over a 5 min time period.

Anthocyanin Encapsulation Efficiency and Leakage
The encapsulation efficiency (EE) of W 1 /O/W 2 emulsions containing either unmodified or amidated pectin as well as the leakage of anthocyanins from the W 1 phase to the W 2 phase was determined. Prepared emulsions were diluted 50% in the background electrolyte then centrifuged at 20,000× g for 15 min. The aqueous phase was carefully removed and filtered through a 0.80 µm cellulose acetate syringe filter (Sartorius, Göttingen, Germany). The aqueous samples were then placed onto 0.22 µm cellulose acetate centrifuge filters (Corning Incorporated, Corning, NY, USA) and centrifuged at 15,500× g for 45 min to remove suspended solids. The clear anthocyanin solutions were then analysed using a ThermEvo UV-Vis spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA) at a wavelength of 520 nm. The anthocyanin concentration was determined from a calibration curve of known concentrations of MEDOX ® (London, UK) (concentration of anthocyanin in the stock material was determined by HPLC, and this analysis is given in the Supplementary Materials). The EE of each emulsion, defined as the percentage of anthocyanins retained within the W 1 phase following emulsion production, was calculated as follows: where TAC is the total anthocyanin content added to the W1 phase and FAC is the free anthocyanin content in the W 2 phase (with 1:1 w/w dilution considered).

Emulsion Microstructure
Confocal laser scanning microscopy (CLSM) (Carl Zeiss AG, Oberkochen, Germany) was used to study the structure of the double emulsions [10,[25][26][27]. Figure 1A,B are images of a W 1 /O/W 2 emulsion, formulated with 0.1 M citrate buffer and amidated pectin in the W 1 phase, on day 1 ( Figure 1B shows a magnified view of the same sample). The oil droplets (red regions) contained a significant amount of aqueous phase, W 1 , as evidenced by the darker unstained spherical regions of varying sizes within the oil droplets. The oil droplets seemed to form 'rafts' of aggregates, consistent with previous studies using soy lecithin and CMCNa [15]. Figure 1C,D show the same emulsion on day 2, where a reduction in the amount of encapsulated W 1 droplets was apparent, suggesting that W 1 droplets are being expelled from the oil phase. The same emulsion on day 5 ( Figure 1E,F) did not appear to differ markedly from the emulsion on day 2; loss of encapsulated W 1 droplets occurred primarily within the first 24 h. In addition, the W 1 droplets contained within the oil phase appear to be smaller on days 2 and 5 than on day 1. The higher conductivity of the W 1 phase compared to the W 2 phase (Table S1, Supplementary Materials) means that there is likely a movement of water from W 2 to W 1 , causing the W 1 droplets to swell. Once these W 1 droplets reach a critical volume, they are they likely to be expelled from the oil droplets. Figure 1E,F (day 5) show differences in the oil droplet shape compared with days   Figure 1 suggest there was significant crossover of oil and water droplets within the size distribution dataset for the 0.1 M citrate buffer emulsions; there were gelled W 1 droplets up to 5 µm in diameter as well as small oil droplets 1 µm in diameter. As such, the two peaks are not strictly representative of separate droplet phases. However, it is likely that the lower and upper regions of the size distributions result primarily from W 1 and oil droplets, respectively, considering the emulsification conditions.  [12,18,28]. The mechanism was reported as either the transport of water molecules from the W 1 droplets to W 2 phase, driven by an osmotic pressure gradient [26], or complete expulsion of W 1 droplets into the W 2 phase [28]. In the case of the 0.1 M citrate buffer and 0.35 M KCl emulsion systems, the conductivity within the W 1 phase was higher than that of the W 2 phase (Table S1), suggesting that the movement of water would likely be from W 2 to W 1 , thus increasing the W 1 droplet size. An increase in the W 1 droplet size resulting from water transport and/or droplet aggregation may explain the upward shift in the lower peaks for both the 0.1 M citrate buffer and 0.35 M KCl emulsions (Figure 2A,C). The size distributions on days 1, 2, and 5 for the 0.1 M citrate emulsion were in keeping with the CLSM data in Figure 1, where the greatest change occurred in the first 24 h of storage, followed by minimal change between days 2 and 5. The smaller droplets showed an increase in size, while the larger (predominantly oil) droplets showed a decrease. These changes in size distribution support a theory of osmotic-driven swelling of the W 1 droplets, followed by subsequent expulsion into the W 2 phase. Coalescence of the smaller oil droplets could also account for the change in size distribution for the lower size region, however, coalescence of the larger oil droplets and subsequent creaming/destabilisation of the emulsions was not seen, indicating good stability of the oil phase.

Droplet Size Analysis
An overall increase was noted for the upper size regions of the 0.1167 M adipic acid and 0.0075 M KCl systems. The size distribution for the 0.1167 M adipic acid system showed a 13.71% increase in upper peak position over the 20-day storage period, from 9.85 to 11.20 µm, while the smaller droplets within the system also seemed to be increase in diameter; the lower peak (0.52 µm) of the distribution decreased in volume while the higher peak (1.45 µm) increased in volume. However, the volume-weighted diameter percentile data for the three 0.1167 M adipic acid emulsions ( Figure S1B) did not provide evidence of a significant increase in d (0.5) or d (0.9). There was a notable increase in d (0.1) from 1.01 ± 0.05 µm to 1.38 ± 0.16 µm. The mechanism for this volume increase for lower peaks is likely due to W 1 droplet aggregation and/or small oil droplet coalescence. Swelling of W 1 is less likely as the conductivity of W 1 was less than that of W 2 . The absence of change in the d (0.5) and d (0.9) values suggests that, unlike the 0.1 M citrate buffer and 0.35 M KCl emulsions, there was either minimal expulsion of gelled W 1 droplets into the W 2 phase or there an overall increase in the size of the larger (predominantly oil) droplets due to coalescence, which offset any decrease that would have otherwise been noticed due to W 1 droplet expulsion. A significant shift in the upper peak was noted for the 0.0075 M KCl system in Figure 2D and confirmed by the volume-weighted diameter percentile data in Figure S1D. The initially narrow distribution for 0.0075 M KCl centred around 6.72 µm shifted upward to 7.63 µm, and an additional shoulder around 27.37 µm appeared ( Figure 2D). The d (0.5) increased from 7.98 ± 1.37 µm to 12.10 ± 1.96 µm and the d (0.9) increased significantly from 20.10 ± 3.22 to 46.00 ± 4.83 µm. The lower peak around 0.46 µm remained relatively consistent. The 0.0075 M KCl system showed significant coalescence between oil droplets during the storage period, but there was little evidence to suggest that any appreciable aggregation or swelling of the W 1 phase was occurring.
The droplet size analysis depicts differences in droplet behaviour as a function of electrolyte composition. For the 0.1 M citrate buffer, 0.1167 M adipic acid, and 0.35 M KCl systems, there was an increase in the size of the smaller droplets (lower size region). The likely explanation is an osmotic pressure-driven transfer of W 2 to W 1 , causing swelling of the internal water droplets. There is also a possibility that coalescence of small oil droplets (seen in Figure 1) causes the increase in the lower peaks for these two systems. The 0.1 M citrate buffer and 0.35 M KCl systems showed a decrease in the size of the larger droplets (upper size region). Expulsion of W 1 droplets caused a decrease in oil droplet size. For the 0.1167 M adipic acid emulsions, no change in the upper peak was noted, suggesting that coalescence between oil droplets may offset any observed decrease in oil droplet size resulting from W 1 droplet expulsion. The 0.0075 M KCl system showed a significant change in oil droplet size distribution that led to eventual destabilisation (creaming) of the W 1 /O/W 2 emulsions, indicating that the lower concentration of electrolyte does not support W 1 /O/W 2 emulsion stability. The nature of the electrolyte also has some bearing on the droplet size evolution following production. In terms of the W 1 phase, this is likely due to the interactions of the electrolyte with pectin. Slight changes in the extent of gelation may influence how the W 1 droplets are formed during the emulsification procedure. According to Frank et al., the addition of a hydrocolloid to the inner water phase affects droplet formation during homogenisation [22]. Thus, any changes to W 1 viscosity due to electrolyte composition may be the cause of the difference in initial W 1 droplet size distribution.

Colour Analysis
The CIE L*a*b* colour parameters were measured for each W 1 /O/W 2 and W 1 /O sample over the 20-day storage period to monitor colour changes for all studied systems. Figure 3 shows the a* (Panel A) and b* (Panel B) parameters for the W 1 /O/W 2 emulsions formulated with different electrolytes as a function of storage time. It is immediately apparent that the a* parameter decreased markedly over the 20-day storage period, consistent with other studies [12,23]. In contrast, colour retention was better in the W 1 /O emulsion and W 1 /O/W 2 emulsions for all electrolyte systems (see Figure S3A)  emulsions showed a period of decline over five and 10 days, respectively, before their b* values began to increase. Anthocyanins are known to degrade to produce yellowish-brown coloured compounds [12,21,29], so the increasing amount of degradation products is likely to contribute to the increase in b* intensity. An increase in b* intensity relative to a* creates an overall shift in colour towards yellow/brown hues (Equation (2)). Similar to the a* values, the b* values for the 0.1 M citrate buffer and 0.1167 M adipic acid W 1 /O emulsions decreased less over 20-days than their W 1 /O/W 2 counterparts ( Figure S3B) To better understand the overall effect of concurrent changes in a* and b*, the colour parameters chroma (c*, also termed colour intensity) and hue angle (h • ) were calculated from Equations (1) and (2), respectively. The c* vs. storage time plots for the W 1 /O/W 2 emulsions in Figure 4A showed a decrease in vibrance for all systems over the 20-day period. The c* analysis for the W 1 /O emulsions is presented in Figure S4A

Rheology
Shear rate ramps (flow curves) were performed on each emulsion for days 1 to 20. All flow curves showed a decrease in viscosity as a function of shear rate, indicating that all systems had non-Newtonian shear-thinning flow behaviour, consistent with other double emulsion studies [16,28,30]. According to McClements, shear-thinning can occur due to altered spatial distribution of particles; non-spherical particle alignment with a flow field; removal of bound solvent molecules; and the deformation of flocs [25]. Flow curves from a single representative emulsion of both the 0.1 M citrate buffer and 0.35 M KCl systems are presented in Figure 5 for days 1 and 20. The results highlight the differences in rheological properties that develop during emulsion storage. At the time of measurement on day 1, the systems behaved similarly to the two datasets in close agreement. However, by the end of the storage period, the nature of the emulsions had changed depending on the electrolyte system. The 0.1 M citrate buffer, 0.35 M KCl, and 0.0075 M KCl emulsions became less viscous over time (Figures 5 and S5). Interestingly, the 0.1167 M adipic acid system showed an increase in viscosity over the first 10 days of storage, followed by a gradual decrease from days 10 to 20 ( Figure S5, only days 1 and 20 shown). Although the viscosity decreased from days 10 to 20, the viscosity was still higher at day 20 than day 1.
To better summarise the effect of storage time on emulsion behaviour, all experimentally obtained flow curves were fitted with the Ostwald de-Waele (power-law) model as a function of shear rate, . γ, as shown in Equation (4): where k is the consistency index and n is the power law exponent. The change in viscosity of the 0.0075 M KCl system over the storage period was not large compared to the other emulsion systems, as highlighted by a decrease in the parameter k from 1.15 ± 0.15 Pa·s n to 0.66 ± 0.13 Pa·s n (shown in Figure 6A). The decrease in viscosity is most likely the result of oil droplet coalescence, as evidenced by the droplet size analysis in Section 3.2. An increase in droplet size of the dispersed phase serves to decrease the viscosity of the system [25,31]. The 0.1 M citrate buffer and 0.35 M KCl systems showed a decrease in viscosity over time. For the 0.1 M citrate buffer system, k decreased from 5.02 ± 1.29 Pa·s n to 2.40 ± 0.34 Pa·s n , while for the 0.35 M KCl emulsions, k decreased from 6.50 ± 1.36 Pa·s n to 3.27 ± 0.16 Pa·s n . The particle size data suggest no appreciable coalescence within the oil phase, meaning that these mechanisms are unlikely to be the underlying cause of the decrease in viscosity. However, the state of aggregation of these suspensions may well vary over time, and this will not always be revealed by particle size measurement of a diluted emulsion (such as the data presented in Figure 2). Based on the rheology data for both the 0.35 M KCl and 0.1 M citrate systems, the emulsions have a lower degree of aggregation as the emulsion ages. The change in viscosity over time for the 0.1167 M adipic acid emulsions was different to that of the other emulsion systems. On day 1, the k parameter was 2.91 ± 0.39 Pa·s n , increasing to 6.85 ± 0.63 Pa·s n on day 10, before decreasing slightly to 5.96 ± 0.35 Pa·s n on day 20. The overall increase in viscosity is likely to be the result of an increase in aggregation of the oil droplets in the emulsion over time, potentially due to some effect of 0.1167 M adipic acid on the emulsifiers in the system, or their interfacial population. Figure 6B shows the change in the power law exponent, n, over time. The n values for the 0.35 M KCl emulsions remained unchanged over the storage period (n = 0.37 ± 0.04 on day 1 and n = 0.37 ± 0.01 on day 20). The 0.1167 M adipic acid emulsions experienced a decrease in n over time, from 0.51 ± 0.02 on day 1 to 0.41 ± 0.01 on day 20. For the 0.0075 M KCl emulsions, n increased slightly from 0.68 ± 0.02 on day 1 to 0.73 ± 0.01 on day 20. Likewise, the n value for 0.1 M citrate buffer increased with time from 0.41 ± 0.05 to 0.58 ± 0.02. An increase in n means that the sample is becoming slightly less shearthinning [31].

Effect of Pectin Chemistry on Anthocyanin Colour and Leakage
The results from Sections 3.1-3.4 indicate that the best performance of the electrolyte systems in terms of W 1 /O/W 2 emulsion stability and anthocyanin colour retention was the 0.1 M citrate buffer system. As such, this electrolyte composition was chosen for further analyses, whereby the pectin chemistry (unmodified or amidated) was analysed for any effects on colour retention and anthocyanin encapsulation efficiency and leakage. Sections 3.1 and 3.2 show a movement of W 1 droplets to the W 2 phase occurring due to W 1 droplet expulsion and, as highlighted in Section 3.3, this is detrimental for colour stability. An analysis was performed to determine the colour retention of anthocyanins in the presence of both unmodified and amidated pectin, and whether the effect is a result of anthocyanin retention within the W 1 phase. Anthocyanin retention within the W 1 phase was determined via Equation (3); UV-Vis was used to quantify anthocyanins in the W 2 phase, which was compared to the amount of anthocyanin added at the time of formulation. The process requires a 50:50 dilution of the W 1 /O/W 2 emulsion with the background electrolyte.
There was a marginal difference in the encapsulation efficiency of anthocyanins due to the type of pectin used to gel the W 1 phase. Unmodified pectin emulsions returned an encapsulation efficiency of 95.0 ± 0.8%, while the amidated pectin returned an encapsulation efficiency of 97.0 ± 0.6%. The results indicate that at the time of production, the amidated pectin allowed for greater retention of anthocyanins within the W 1 droplets. This difference could be a result of more extensive gelation within the amidated pectin system or increased binding of anthocyanins to amidated pectin. Figure 7 shows the percentage of anthocyanins (added to the W 1 phase at the time of formulation) present within the W 2 phase as a function of time and pectin type. Initially, there is a difference between the two pectin types, with pectin amide (3.0 ± 0.6%) yielding a lower concentration of anthocyanins in the W 2 phase than unmodified pectin (5.0 ± 0.8%). The greatest change in anthocyanin leakage from W 1 to W 2 occurred over the first 24 h of storage. This leakage of anthocyanins during the first 24 h aligns with our analysis of the CLSM images in Figure 1 and the droplet size distribution data in Figure 2A. During the first 24 h, we saw the greatest extent of W 1 droplets being expelled into the W 2 phase. Anthocyanin content within the W 2 phase peaked on day 5 for unmodified pectin (15.8 ± 0.9%) and day 15 for amidated pectin (13.9 ± 1.1%), suggesting slower leakage of anthocyanins due to the presence of amidated pectin. However, as time elapsed, the difference in anthocyanin leakage between the two pectin types became less clear: when at day 20, the amount of anthocyanin in the W 2 phase was identical for both systems (12.8 ± 0.1% for amidated pectin and 12.7 ± 0.5% for unmodified pectin). The average leakage values were lower for amidated pectin, however, the results were skewed by a single pectin amide emulsion having far greater encapsulation stability. Given the sample size of n = 3, there is no conclusive proof that amidated pectin is beneficial in terms of preventing anthocyanin leakage from the W 1 to W 2 phases.  Figure 8C). Initially, the c* value for amidated pectin emulsions was 25.52 ± 0.22, marginally higher than that of unmodified pectin emulsions at 24.85 ± 0.41. By day 20, there was no significant difference in the c* values, meaning that the amidated pectin emulsions experienced a greater decrease in c* (a decrease from 25.5 on day 1 to 16 on day 20) than the unmodified pectin emulsions (a decrease from 24.5 at day 1 to 16 on day 20). The differences in a* and b* ( Figure 8A,B) between the two pectin systems caused a subsequent difference in h • ( Figure 8D), with the unmodified pectin system having lower values to that of the amidated pectin system. The h • values decreased (from initial values of 24.52 ± 0.60 • for amidated pectin emulsions and 23.5 ± 0.40 • for unmodified pectin emulsions) until around day 15 when the values began to increase. The increase in h • resulted from the change in b* being less pronounced compared with that of a* (Equation (2)). At day 20, the h • values were 21.08 ± 0.21 • for amidated pectin emulsions and 18.89 ± 0.04 • for unmodified pectin emulsions. In terms of W 1 /O/W 2 emulsions, there was little difference in the a* and c* parameters for the unmodified and amidated pectin systems over the 20-day storage period. However, differences in the b* parameter also resulted in noticeable changes to h • . The differences in colour parameters for the W 1 /O emulsions formulated with either amidated or unmodified pectin were less noticeable than that of the W 1 /O/W 2 emulsions. The magnitude and change in the parameters as a function of storage time differed between the W 1 /O and W 1 /O/W 2 emulsions, similar to the results in Section 3.4. In terms of a*, there was little difference between the two W 1 /O formulations with the amidated pectin emulsions experiencing a decrease in a* from 21.98 ± 0.30 to 18.27 ± 0.56 (a decrease of 16.90%), and the unmodified pectin emulsions experiencing a decrease from 21.56 ± 0.10 to 17.80 ± 0.20 (a decrease of 17.44%). Additionally, there was little difference in b*; the amidated pectin emulsions decreased from 12.03 ± 0.38 to 10.96 ± 0.48 (8.92% decrease) and the unmodified pectin emulsions decreased from 11.49 ± 0.20 to 10.42 ± 0.15 (9.31% decrease). The absence of any noticeable difference between the a* and b* parameters of the two emulsion formulations meant there was no significant difference between either the c* or h • values over the 20-day storage period.
Analysis of anthocyanin colour retention yielded relatively few differences between emulsions formulated with amidated pectin or unmodified pectin in the W 1 phase. For W 1 /O/W 2 emulsions, the main point of difference between the two pectin systems was the b* parameter, which was lower overall for unmodified pectin emulsions. This, in turn, affected the h • values and signified a minor difference in the colour produced by each emulsion. Taking into account the anthocyanin leakage from the W 1 to W 2 phases, as shown in Figure 7, there is not enough evidence to suggest that either amidated or unmodified pectin has any benefit in the stabilisation of anthocyanins within the formulated W 1 /O/W 2 emulsion systems tested.
The differences in colour parameters for the W 1 /O emulsions ( Figure 8) formulated with either amidated or unmodified pectin were less noticeable than that of the W 1 /O/W 2 emulsions. The magnitude and change in the parameters as a function of storage time differed between the W 1 /O and W 1 /O/W 2 emulsions, similar to the results in Section 3.4. In terms of a*, there was little difference between the two W 1 /O formulations, with the amidated pectin emulsions experiencing a decrease in a* from 21.98 ± 0.30 to 18.27 ± 0.56 (a decrease of 16.90%), and the unmodified pectin emulsions experiencing a decrease from 21.56 ± 0.10 to 17.80 ± 0.20 (a decrease of 17.44%). Additionally, there was little difference in b*; the amidated pectin emulsions decreased from 12.03 ± 0.38 to 10.96 ± 0.48 (8.92% decrease) and the unmodified pectin emulsions decreased from 11.49 ± 0.20 to 10.42 ± 0.15 (9.31% decrease). The absence of any noticeable difference between the a* and b* parameters of the two emulsion formulations means that there was no significant difference between either the c* or h • values over the 20-day storage period. In terms of W 1 /O emulsions, there was no difference in the colour retention of the two systems (i.e., there is no difference in the ability of the two pectin varieties to stabilise anthocyanins within W 1 /O emulsions).

Conclusions
The results of this study demonstrate the significant differences in anthocyanin and emulsion stability arising from the electrolyte phase composition in single and double emulsions. This was made apparent from the colour analysis of both water-in-oil (W 1 /O) emulsions and water-in-oil-in-water (W 1 /O/W 2 ) emulsions, highlighting the need to understand the influence of aqueous phase composition on overall double emulsion stability (and precursor single emulsion stability) before determining the ability of complex emulsions to protect encapsulated molecules. Droplet sizing and rheology data revealed the differences in emulsion stability as a function of electrolyte composition; an electrolyte phase consisting of 0.1 M citrate buffer allowed for the best performance in terms of anthocyanin colour retention in W 1 /O and W 1 /O/W 2 emulsions as well as stable droplet size and emulsion rheology. While the electrolyte composition effects were clear, there was no significant influence of pectin chemistry on the stability and protection of anthocyanins.
Supplementary Materials: The following are available online at https://www.mdpi.com/article/10 .3390/foods11010034/s1, Table S1: A summary of the pH and conductivity values of the background electrolyte, W 1 and W 2 solutions for each composition. Conductivity is in mS.cm −1 . Table S2: Quantitative analysis of major anthocyanins in MEDOX ® expressed as cyanidin-3-glucoside equivalents.  Figure S2: A schematic of the CIEL*a*b* colour system, highlighting the parameters relevant to this work, namely: a*, b*, c* and h • , Figure S3: The CIEL*a*b* colour parameters a* (Panel A) and b* (Panel B) for W 1 /O emulsions. The 0.1 M citrate buffer system is represented by circles, 0.1167 M adipic acid by squares, 0.35 M KCl by triangles, and 0.0075 M KCl by diamonds. Figure S4: Chroma (c*, Panel A) and hue angle (h • , Panel B) for W 1 /O emulsions calculated from the data in Figure S3. The 0.1 M citrate buffer system is represented by circles, 0.1167 M adipic acid by squares, 0.35 M KCl by triangles, and 0.0075 M KCl by diamonds. Figure S5: Flow curves between shear rates of 1 and 100 s −1 for 0.1167 M adipic acid (red squares) and 0.35 M KCl (purple diamonds) emulsions on days 1 (closed symbols) and 20 (open symbols). Figure S6: Digital photograph of the formed double emulsions, made using amidated pectin (left sample has a higher concentration of NaCMC, which was not used for the data presented in this work).  Institute, University of South Australia, a facility funded by the University, and South Australian and Australian Federal Governments.

Conflicts of Interest:
The authors declare no conflict of interest.